EP1895016A1 - Verfahren zur Ermittlung von Arzneimittelempfindlichkeit durch Analyse von GIRK-Kanal-Genen - Google Patents

Verfahren zur Ermittlung von Arzneimittelempfindlichkeit durch Analyse von GIRK-Kanal-Genen Download PDF

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EP1895016A1
EP1895016A1 EP07017086A EP07017086A EP1895016A1 EP 1895016 A1 EP1895016 A1 EP 1895016A1 EP 07017086 A EP07017086 A EP 07017086A EP 07017086 A EP07017086 A EP 07017086A EP 1895016 A1 EP1895016 A1 EP 1895016A1
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gene
gene polymorphism
polymorphism
haplotype
oligonucleotide
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EP1895016B1 (de
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Kazutaka Ikeda
Masakazu Hayashida
Daisuke Nishizawa
Ichiro Sora
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Tokyo Metropolitan Organization for Medical Research
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    • C12Q1/00Measuring or testing processes involving enzymes, nucleic acids or microorganisms; Compositions therefor; Processes of preparing such compositions
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    • C12Q1/6876Nucleic acid products used in the analysis of nucleic acids, e.g. primers or probes
    • C12Q1/6883Nucleic acid products used in the analysis of nucleic acids, e.g. primers or probes for diseases caused by alterations of genetic material
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    • C12Q2600/00Oligonucleotides characterized by their use
    • C12Q2600/156Polymorphic or mutational markers
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    • C12BIOCHEMISTRY; BEER; SPIRITS; WINE; VINEGAR; MICROBIOLOGY; ENZYMOLOGY; MUTATION OR GENETIC ENGINEERING
    • C12QMEASURING OR TESTING PROCESSES INVOLVING ENZYMES, NUCLEIC ACIDS OR MICROORGANISMS; COMPOSITIONS OR TEST PAPERS THEREFOR; PROCESSES OF PREPARING SUCH COMPOSITIONS; CONDITION-RESPONSIVE CONTROL IN MICROBIOLOGICAL OR ENZYMOLOGICAL PROCESSES
    • C12Q2600/00Oligonucleotides characterized by their use
    • C12Q2600/172Haplotypes

Definitions

  • the present invention relates to a method of evaluating drug sensitivity by analyzing GIRK channel genes.
  • the pain sensation plays an important role in terms of a biological warning system, however, excessive pain significantly decreases QOL (quality of life) unless it is properly controlled.
  • QOL quality of life
  • GIRK channel G protein-activated inwardly rectifying potassium channel
  • the present invention provides a method of predicting an individual difference in drug sensitivity or disease vulnerability, more specifically, drug sensitivity or disease vulnerability associated with the required number of administration of analgesics, total amount of analgesics, vulnerability to drug dependence, prolongation of stimulant-induced psychosis or the like using GIRK channel gene polymorphisms.
  • the present inventors paid attention to GIRK channel genes and made intensive studies based on past findings and clinical data. As a result, they identified several useful gene polymorphisms by analyzing a correlation between various GIRK channel gene polymorphisms and drug sensitivity or disease vulnerability to analgesics and stimulants. They also found a linkage disequilibrium among these identified gene polymorphisms and revealed a significant correlation with drug sensitivity or disease vulnerability.
  • the present invention is as follows: ⁇ 1> A method of evaluating drug sensitivity, which comprises linking a gene polymorphism in the GIRK channel genes or a haplotype comprising the gene polymorphism to individual drug sensitivity. ⁇ 2> The method as described in ⁇ 1> above, which comprises the steps of:
  • Narcotic analgesics typified by morphine act on a protein called an opioid receptor thereby to cause analgesia.
  • opioid receptors There are three types of opioid receptors: mu, delta and kappa ( ⁇ , ⁇ , ⁇ ), and all receptors are involved in an analgesic action. These receptors are Gi/o protein-coupled receptors, therefore, they not only inhibit adenylate cyclase and calcium channels via a Gi/o protein, but also activate GIRK channels.
  • the GIRK channel is an ion channel having an important function in regulating excitability of neurons and heart rate and is present in large quantities in the brain and heart.
  • the GIRK channel penetrates the cell membrane twice at M1 and M2 regions and has a structure in which H5 region located between the M1 and M2 regions projects into the cell membrane.
  • the H5 region forms a central portion through which ions pass.
  • the GIRK channel functions as a tetramer composed of four subunits. There are four types of subunits: GIRK1, GIRK2, GIRK3 and GIRK4. In the brain, GIRK1, GIRK2 and GIRK3 subunits are strongly expressed, and a GIRK1/2 channel by the combination of GIRK1 and GIRK2 subunits mainly functions therein. Incidentally, in the heart, GIRK1 and GIRK4 subunits are strongly expressed, and a GIRK1/4 channel mainly functions therein.
  • the present inventors identified gene polymorphisms (such as SNP) of GIRK2 and GIRK3 subunits, which are expressed strongly in the brain among the four subunits capable of constituting GIRK channels in healthy subjects (Figs 1 and 2). Further, a linkage disequilibrium analysis was carried out as needed, and a block exhibiting a strong linkage disequilibrium (a haplotype block) was identified.
  • SNP gene polymorphisms
  • the linkage equilibrium means to a case where the relationship between two gene polymorphisms on the chromosome is independent
  • the linkage disequilibrium means a case where a gene polymorphism is linked to the other gene polymorphism thereby deviating from the equilibrium situation according to Mendel's law of independence
  • the haplotype means a genetic structure of such as genes or gene polymorphisms located in the vicinity of each other in one allele of a set of alleles (a gene derived from one of the parents).
  • haplotype also refers to a combination of the arrangement of the same gene in this haplotype block.
  • the present inventors analyzed the GIRK2 subunit gene, and as a result, they found five gene polymorphisms (A-1361G, G1250A, T-244C, C-227T and A-68G) in the 5' flanking region, one gene polymorphism (IVS1C75167T) in a portion of intron, and one gene polymorphism each (three gene polymorphisms in total: A1032G, C1569T and C1843G) in the coding region of exon 3, the coding region of exon 4 and the 3' noncoding region (see Fig. 1).
  • a gene polymorphism with a high minor allele frequency in the exons was A1032G.
  • GIRK3 subunit gene found four gene polymorphisms (A-1329C, C979G, C-968G and A-447G) in the 5' flanking region, two gene polymorphisms (C1211T and C1339T) in the coding region of exon 3, and four gene polymorphisms (C1781T, C1817T, G2069A and C2429T) in the 3' noncoding region (see Fig. 2).
  • gene polymorphisms with a particularly high minor allele frequency in the exons were C1339T, C1781T and the like, and further, a gene polymorphism with an amino acid substitution was only C1339T.
  • an individual difference in drug sensitivity or disease vulnerability such as the required number of administration of analgesics, total amount of analgesics, vulnerability to drug dependence or prolongation of stimulant-induced psychosis can be easily evaluated.
  • the results of evaluating drug sensitivity or disease vulnerability can be important information for determining the administration number, amount, type or the like of drugs to be administered to an individual, and predicting side effects.
  • the present invention is extremely useful for personalized pain therapy or drug dependence therapy.
  • the human GIRK channel gene polymorphisms of the present invention include mainly single nucleotide polymorphisms (hereinafter also referred to as SNP), however it is not limited to this, and insertion polymorphisms, deletion polymorphisms, and nucleotide repeat polymorphisms can also be included.
  • SNP single nucleotide polymorphisms
  • the single nucleotide polymorphism means a gene polymorphism caused by substitution of a specific one nucleotide of a gene with another nucleotide.
  • the insertion/deletion polymorphism means a gene polymorphism caused by deletion/insertion of one or more nucleotides.
  • nucleotide repeat polymorphism means a gene polymorphism caused by a difference in the number of repeats of nucleotide sequence.
  • the nucleotide repeat polymorphism is divided into a microsatellite polymorphism (the number of nucleotides: about 2 to 4 nucleotides) and a VNTR (variable number of tandem repeat) polymorphism (repeated nucleotides: several to several tens of nucleotides) according to the difference in the number of repeated nucleotides, and the number of repeats varies depending on individuals.
  • the information of human GIRK channel gene polymorphisms (SNPs in GIRK2 and GIRK3 observed on the genome of Japanese healthy subjects) elucidated by the present invention is shown in Table 3.
  • the gene polymorphisms shown in Table 3 are included in the GIRK channel gene polymorphisms of the present invention.
  • GIRK2 indicates the GIRK2 subunit gene.
  • GIRK2 gene is also referred to as Kir3.2 gene and sometimes represented by “KCNJ6” (italic form)
  • GIRK3 gene is also referred to as Kir3.3 gene and sometimes represented by "KCNJ9” (italic form).
  • Porition means a position on the genome of a GIRK channel gene, and indicates a 5' flanking region, as well as each exon and intron.
  • Gene polymorphism name is the name of SNP at a position on the genome and given by the present inventors. Basically, an alphabet of A, G, C or T is given before and after two- to five-digit number and symbol, respectively, thus which nucleotide is involved in SNP can be identified.
  • A-1361G indicates a gene polymorphism in which the nucleotide located 1361 bp upstream (5' side) of the transcription start site is changed between A and G.
  • C1339T indicates a gene polymorphism in which the nucleotide located 1339 bp downstream (3' side) of the transcription start site is changed between C and T.
  • nucleotide at the transcription start site when the nucleotide at the transcription start site is determined to be 1, the nucleotide located one nucleotide upstream of the transcription start site is determined to be -1 and the nucleotide located one nucleotide downstream of the transcription start site is determined to be 2. In the same manner, the nucleotides are counted sequentially.
  • IVS1C75167T in the column of "Intron 1" indicates a gene polymorphism in intron 1, in which the nucleotide at the start site in intron 1 is determined to be 1, and the nucleotide located 75167 bp downstream thereof is changed between C and T.
  • Major allele indicates an allele occurring in the majority of the genomes of Japanese healthy subjects
  • minor allele indicates an allele occurring in the minority of the genomes of Japanese healthy subjects.
  • a method of obtaining gene polymorphism information is as follows, for example.
  • the present invention provides an oligonucleotide which contains any one of GIRK2 subunit gene polymorphisms (A-1361G, G-1250A, T-244C, C-227T, A-68G, IVS1C75167T, A1032G, C1569T and C1843G) and GIRK3 subunit gene polymorphisms (A-1329C, C-979G, C-968G, A-447G, C1211T, C1339T, C1781T, C1817T, G2069A and C2429T), and is capable of being specifically hybridized to a DNA fragment containing a gene polymorphism in the GIRK channel genes.
  • the gene polymorphic site is the 51st nucleotide in the nucleotide sequence represented by any one of SEQ ID NOS: 1 to 19.
  • the oligonucleotide of the present invention has at least 10 nucleotides, preferably 10 to 150 nucleotides, more preferably 10 to 45 nucleotides, further more preferably 14 to 25 nucleotides.
  • oligonucleotide of the present invention examples include oligonucleotides having a nucleotide sequence represented by any one of SEQ ID NOS: 1 to 19 containing the above-mentioned gene polymorphism or a nucleotide sequence complementary to the nucleotide sequence (Table 4).
  • the oligonucleotides of the present invention can be used as a probe or a primer specific to a GIRK channel gene in the detection of GIRK channel gene polymorphism described in the below-mentioned 5.
  • Table 4 Gene name Position Gene polymorphism name Sequence SEQ ID NO GIRK2 5' flanking region A-1361G 1 G-1250A 2 T-244C 3 C-227T 4 A-68G 5 Intron 1 IVS1C75167T 6 Exon 3 A1032G 7 Exon 4 C1569T 8 C1843G 9 GIRK3 5' flanking region A-1329C 10 C-979G 11 C-968G 12 A-447G 13 Exon 3 C1211T 14 C1339T 15 C1781T 16 G1817T 17 G2069A 18 C2429T 19
  • a haplotype by using SNP among the above-mentioned gene polymorphisms, a haplotype can be constructed.
  • the SNP to become a target of a haplotype analysis may be any as long as its gene polymorphism frequency is 0.5% or higher, preferably, those with a gene polymorphism frequency of 1%, more preferably those with a gene polymorphism frequency of 5% or higher can be selected. Further, SNP to become a target of a haplotype analysis may be a full or partial sequence thereof.
  • the haplotype analysis can be carried out using various computer programs, and for example, Haplotype Estimation (available from the website: http://www.bioinf.mdc-berlin.de/projects/hap/: Rohde K, Fuerst R: Haplotyping and estimation of haplotype frequencies for closely linked biallelic multilocus genetic phenotypes including nuclear family information. Max-Delbrueck-Centrum for Molecular Medicine, Berlin, Germany) can be used.
  • haplotype analysis with regard to the 9 sites of SNPs which are GIRK2 subunit gene polymorphisms and the 10 sites of SNPs which are GIRK3 subunit gene polymorphisms among the GIRK channel gene polymorphisms in Japanese healthy subjects found as in the above-mentioned 2, a haplotype was estimated using Haplotype Estimation. The estimated haplotypes are shown in Tables 5 and 6. Table 5 Gene name: GIRK2 Gene polymorphism name Haplotype No.
  • a haplotype frequency in the population is calculated, and a linkage disequilibrium analysis can be carried out based on the thus obtained haplotype frequency.
  • the D' value and r 2 value, which indicate measures of linkage disequilibrium, can be calculated based on the following definition. Definition:
  • SNP A and SNP B there are SNP A and SNP B, and the respective alleles are represented by A and a, and B and b.
  • the four haplotypes formed by SNP A and SNP B are represented by AB, Ab, aB and ab, and the respective haplotype frequencies are represented by P AB , P Ab , P aB and P ab .
  • a haplotype block can be estimated from the results of the linkage disequilibrium analysis.
  • a linkage block can be estimated from the results of the haplotype analysis by using, for example, Haploview (which is accessible from http://www.broad.mit. edu/mpg/haploview/index.php).
  • the information of SNPs indirectly linked to each other in the same block can be obtained. That is, when a gene polymorphism of the GIRK channel (specifically, GIRK2 or GIRK3 subunit) gene is examined, it is not necessary to analyze all the SNPs, and it is only necessary to perform typing for several specific SNPs.
  • GIRK channel specifically, GIRK2 or GIRK3 subunit
  • GIRK channel gene polymorphism when a gene polymorphism occurs in the GIRK channel gene, the function or expression level of GIRK channel might change. Therefore, there is a correlation between a GIRK channel gene polymorphism and various phenotypes associated with the GIRK channel in some cases.
  • a phenotype associated with sensitivity to drugs drug sensitivity
  • a phenotype associated with occurrence of a disease disease vulnerability
  • drug sensitivity an efficacy of drugs, a side effect of drugs, duration of efficacy of drugs and the like
  • disease vulnerability pain sensitivity, vulnerability to drug dependence and the like can be exemplified.
  • the drugs is preferably drugs associated with GIRK, and examples thereof include various drugs acting directly or indirectly on the GIRK channel.
  • examples of the various drugs acting directly or indirectly on the GIRK channel include a GIRK channel function modulator, an opioid receptor function modulator and the like, and preferred is a GIRK channel function modulator.
  • Specific examples thereof include a stimulant such as methamphetamine, a dopamine receptor agonist, a dopamine receptor antagonist, a ⁇ -, ⁇ -, or ⁇ -opioid receptor agonist, a ⁇ -, ⁇ -, or ⁇ -opioid receptor antagonist and the like.
  • GIRK channel function modulator examples include morphine, DAMGO, codeine, methadone, carfentanil, fentanyl, heroin, naloxone, naltrexone, nalorphine, levallorphan, pentazocine, pethidine, buprenorphine, oxycodone, hydrocodone, levorphanol, etorphine, dihydroetorphine, hydromorphone, oxymorphone, tramadol, diclofenac, indomethacin, flurbiprofen axetil, marcain, ethanol, methanol, propanol, butanol, flupirtine, laughing gas, F3 (1-chloro-1,2,2-trifluorocyclobutane), halothane, estradiol, dithiothreitol, thioridazine, pimozide, fluoxetine, paroxetine, desipramine, imipramine, imi
  • morphine, pentazocine, pethidine, buprenorphine, diclofenac, indomethacin, flurbiprofen axetil and marcain are preferred, and morphine, fentanyl and pentazocine are more preferred.
  • mu-opioid receptor function modulator examples include methamphetamine, methylenedioxymethamphetamine, amphetamine, dextroamphetamine, dopamine, morphine, DAMGO, codeine, methadone, carfentanil, fentanyl, heroin, cocaine, naloxone, naltrexone, nalorphine, levallorphan, pentazocine, buprenorphine, oxycodone, hydrocodone, levorphanol, etorphine, dihydroetorphine, hydromorphone, oxymorphone, ethanol, methanol, diethyl ether, tramadol and the like.
  • methamphetamine, morphine, pentazocine and buprenorphine are preferred, and morphine, fentanyl and pentazocine are more preferred.
  • the correlation between a GIRK channel gene polymorphism and a phenotype can be examined as described in the following (1) to (4), for example.
  • test subjects are classified into groups depending on the difference in phenotypes, and comparison of gene polymorphism frequencies or genotypes between healthy subjects and test subjects can be carried out for each group.
  • the phenotype associated with the occurrence of a disease is a stimulant-induced psychotic-like symptom
  • it can be classified, for example, according to a period of time from the start of the use of a stimulant to the occurrence of delusion or hallucination, a period of duration of delusion or hallucination after termination of the use thereof, the presence or absence of the relapse, and the presence or absence of multiple drug abuse.
  • gene polymorphism is affected by the race, birthplace or the like, therefore, it is preferred that in a group showing a similar gene polymorphism to that of a population used for finding an associated gene polymorphism (such as SNP), the above-mentioned evaluation using the gene polymorphism is carried out.
  • the correlation between a GIRK channel gene polymorphism and a phenotype analyzed can be used as an index in a method of predicting sensitivity to various drugs associated with the GIRK channel, a method of selecting a method of treating or preventing a disease associated with the GIRK channel, a method of determining an appropriate administration amount of therapeutic drugs, a method of predicting side effects or the like.
  • the gene polymorphism or the method of the present invention it is possible to evaluate drug sensitivity or disease vulnerability in different races.
  • the subjects are not particularly limited and examples thereof include Japanese, Europeans, Americans and the like, however, in the present invention, they are preferably Japanese or those having a similar gene polymorphism tendency to that of Japanese.
  • genomic DNA is purified from a specimen such as the blood, saliva, skin or the like collected from a human using the phenol method or the like.
  • a commercially available genomic DNA extraction kit such as GFX Genomic Blood DNA Purification Kit (manufactured by GE Healthcare Bio-Sciences KK) or a device may be used.
  • mRNA or total RNA may be extracted instead of genomic DNA.
  • the above-mentioned oligonucleotide of the present invention can be used as a probe or a primer.
  • an example of the gene polymorphism detection method will be described.
  • a high fidelity DNA polymerase for example, KOD Dash polymerase (manufactured by TOYOBO) is used.
  • a primer to be used is designed such that a target SNP in the test sample can be amplified and synthesis is carried out. It is preferred that a gene polymorphism or a strand complementary thereto is contained at a given position between the forward and reverse primers. After completion of the amplification reaction, detection of the amplified products is carried out, and the presence or absence of a gene polymorphism is determined.
  • Table 7 Gene name Position Gene polymorphism name Primer sequence for PCR amplification (5' >3') SEQ ID NO GIRK2 5' flanking region G-1250A CAGGCATTGTGGAGCACGTATTAC 20 CACCCCCTCTTTTTCTTATGGTCA 21 Exon 3 A1032G TTCTCAATAGAGACAGAAACCACCATTGGTTATGGCTACCGGGTCATGA CAGATAAATGT 22 GACACCAGAAACAGACGGTCATC 23 GIRK3 Exon 3 C1339T TTGGGGCAAATGGAGAAGACACGAG 24 GGACCCCTCCCTTCCATACTGGTTT 25
  • the gene polymorphism of the present invention can also be detected by a sequencing method based on the dideoxy method.
  • a sequencer to be used for the sequencing a commercially available ABI series (Applied Biosystems) can be used.
  • a DNA microarray is a microarray in which oligonucleotide probes have been immobilized on a support, and includes a DNA chip, a Gene chip, a microchip, a bead array and the like.
  • a polynucleotide of a test sample is isolated and amplified by PCR, and then labeled with a fluorescent reporter group. Then, a labeled DNA/mRNA, or total RNA is incubated along with an array.
  • this array is inserted in a scanner, and a hybridization pattern is detected.
  • the data of the hybridization is collected as emitted light from the fluorescent reporter group bound to the probe array (i.e., incorporated in a target sequence).
  • a probe which is completely identical with the target sequence generates a stronger signal than those having a region which is not identical with the target sequence. Because the sequence and the position of each probe on the array are known, the sequence of the target polynucleotide reacted with the probe array can be determined based on the complementarity.
  • the TaqMan PCR method is a method utilizing an allele specific oligonucleotide (also referred to as TaqMan probe) labeled with fluorescence and PCR with Taq DNA polymerase.
  • the allele specific oligonucleotide is an oligonucleotide containing a gene polymorphic site.
  • the allele specific oligonucleotide to be used in the TaqMan PCR method can be designed based on the above-mentioned gene polymorphism information.
  • the invader method is a method of detecting a gene polymorphism by subjecting an allele specific oligonucleotide and a template to hybridization.
  • a kit for carrying out the invader method is commercially available (for example, Nano Invader® Array (manufactured by BML, Inc.)), and it is possible to easily detect a gene polymorphism by this method.
  • the present invention provides a kit for evaluating drug sensitivity or disease vulnerability.
  • the kit for detecting a gene polymorphism of the present invention includes one or more components necessary for carrying out the present invention.
  • the kit of the present invention preferably includes a component for storing or supplying an enzyme and/or a reaction component necessary for detecting a gene polymorphism.
  • a component is not limited, however, examples thereof include the oligonucleotide of the present invention, an enzyme buffer solution, dNTP, a reagent for control (such as a tissue sample or a target oligonucleitide for a positive or negative control), a reagent for labeling and/or detection, a solid phase support, a written instruction manual and the like.
  • the kit of the present invention may be a partial kit including only a part of the necessary components. In this case, a user can prepare the other components.
  • the kit of the present invention can be provided as a microarray in which the above-mentioned oligonucleotide has been immobilized on a support.
  • the microarray is one in which the oligonucleotide of the present invention has been immobilized on a support, and includes a DNA chip, a Gene chip, a microchip, a bead array and the like.
  • the kit of the present invention preferably includes an oligonucleotide which contains a GIRK channel gene polymorphism found in the present invention and is capable of being specifically hybridized to a DNA fragment containing the gene polymorphism.
  • the blood is collected before drugs are applied to patients or the like (for example, before surgery, at the time of occurrence of cancer pain or the like), and DNA containing a GIRK channel 1 gene is isolated. Then, IF this gene is reacted with an oligonucleotide in the kit, whereby a genotype is determined.
  • the kit of the present invention may include a primer composed of a nucleotide sequence represented by any one of SEQ ID NOS: 20 to 25 to be used in the detection of a GIRK channel gene polymorphism.
  • the detection of a GIRK channel gene polymorphism using the primer is carried out by, for example, PCR.
  • a dosage regimen such as the type or dose of the drugs can be designed.
  • an effect of the drugs suitable for an individual can be obtained, which is useful in the personalized medicine.
  • morphine it becomes possible to obtain an analgesic effect suitable for an individual, and also to suppress the side effects to the minimum.
  • Genomic DNA was extracted from the blood or the oral mucosa of humans (48 Japanese healthy subjects) by a standard method, and gene polymorphisms were identified in two subunits (GIRK2 and GIRK3) which were strongly expressed mainly in the brain among four subunits of human G protein-activated inwardly rectifying potassium channel
  • the GIRK2 subunit gene includes four exons, and three gene polymorphisms in total, i.e., one gene polymorphism in each of a coding region of exon 3, a coding region of exon 4 and a 3'noncoding region of exon 4 were identified in the Japanese samples. Further, five gene polymorphisms were found in the 5' flanking region, and one gene polymorphism was found in the intron (see Fig. 1 and Table 8).
  • the GIRK3 subunit gene includes three exons, and two gene polymorphisms in the coding region of exon 3, four gene polymorphisms in the 3'noncoding region of exon 3, and four gene polymorphisms in the 5" flanking region were identified in the Japanese samples (see Fig. 2 and Table 8).
  • gene polymorphisms with a particularly high minor allele frequency in the exons were C1339T, C1781T and the like, and a gene polymorphism with an amino acid substitution was only C1339T.
  • “Reported allele” indicates an allele of the sequence registered in GenBank.
  • “Amino acid substitution” means that the type of amino acid after translation is changed depending on the gene polymorphism allele.
  • “Ala366Val” indicates that the amino acid at the position 366 from the N terminus of the peptide chain after translation is substituted with alanine or valine.
  • the symbol “-” means that the type of amino acid is not changed even in any allele.
  • minor allele frequency means the ratio of a minor allele.
  • Numberer of test subjects means the number of healthy subjects to become test subjects.
  • haplotype analysis with regard to the 9 sites of SNPs which are GIRK2 subunit gene polymorphisms and the 10 sites of SNPs which are GIRK3 subunit gene polymorphisms shown in Table 8 among the GIRK channel gene polymorphisms in Japanese healthy subjects, a haplotype is estimated using Haplotype Estimation. The estimated haplotypes are shown in Tables 9 and 10. Table 9 Gene name: GIRK2 Gene polymorphism name Haplotype No.
  • haplotype No. 10 As shown in Table 9, at least 14 haplotypes were estimated as the haplotype of GIRK2 subunit gene polymorphism in the Japanese healthy subjects, and among these, there were 9 haplotypes observed at a high frequency of 3% or higher (haplotype No. 1 to No. 9). Incidentally, 5 or more haplotypes which are estimated to occur at a frequency of less than 3% are collectively shown in haplotype No. 10 in Table 9.
  • haplotypes were estimated as the haplotype of GIRK3 subunit gene polymorphism in the Japanese healthy subjects, and among these, there were 5 haplotypes observed at a high frequency of 3% or higher (haplotype No. 1 to No. 5).
  • a linkage disequilibrium block was estimated from the results of the linkage disequilibrium analysis (Tables 11 and 12) using Haploview (which is accessible from http://www.broad.mit.edu/mpg/haploview/index.php).
  • an r 2 value which is a more stringent index of the linkage disequilibrium, is calculated in the same manner, and the resulting value is written in the cell at the intersection of the column of SNP1 and the row of SNP2 (lower left side of the table).
  • a linkage disequilibrium block was estimated from the results of the linkage disequilibrium analysis (Tables 11 and 12) using Haploview (which is accessible from http://www.broad.mit.edu/mpg/haploview/ index.php).
  • Haploview which is accessible from http://www.broad.mit.edu/mpg/haploview/ index.php.
  • SNP in the GIRK2 subunit gene shown in Table 11 one linkage disequilibrium block containing G-1250A as a Tag SNP was confirmed.
  • SNP in the GIRK3 subunit gene shown in Table 12 a total of two linkage disequilibrium blocks were confirmed in the 5' flanking region and 3' noncoding region of exon 3.
  • Genomic DNA was extracted from the blood or the oral mucosa of 123 patients undergoing surgery, and one gene polymorphism (A1032G) in the GIRK2 subunit gene was determined. Then, a correlation between these results of determination of the gene polymorphism and the required number of administration of analgesics and the total amount of analgesics was analyzed.
  • analgesics such as pentazocine and pethidine, which are mainly administered intravenously, buprenorphine, diclofenac and indomethacin, which are mainly administered as a suppository, flurbiprofen axetil, which is injected by intravenous infusion, as well as epidural morphine and marcain were used.
  • the total amount of analgesics in terms of pentazocine means the total amount of analgesics (mg) in the case where the amount of each administered analgesic is converted to a value corresponding to the potency equivalent to pentazocine.
  • the conversion of the amount of each analgesic to a value corresponding to the potency of pentazocine was carried out by setting a potency equivalent to pentazocine to 35 mg in the case of pethidine (Opystan), 0.4 mg in the case of buprenorphine (Lepetan), 100 mg in the case of diclofenac (Voltaren), 100 mg in the case of flurbiprofen axetil (Ropion), 2 mg in the case of epidural morphine, and 20 ml in the case of marcain (0.5%).
  • GIRK2 subunit gene polymorphism A correlation between the GIRK2 subunit gene polymorphism and the required number of administration of analgesics was examined.
  • the data to be analyzed was the same as in Example 2.
  • the total amount of analgesics was significantly larger compared with a group of patients who had either one of the major alleles or a group of patients who had both major alleles.
  • genomic DNA was extracted from the blood of 197 methamphetamine-dependent patients and 360 healthy subjects, and the GIRK3 subunit gene polymorphism (C1339T) was determined. The results are shown in the following Table 17.
  • a group of patients with prolonged stimulant-induced psychosis (for one month or more) and a group of healthy subjects were compared.
  • the results are shown in the following Table 18.
  • the methamphetamine-dependent patients were classified into two groups: a group of early disappearance type in which the period of duration of delusion or hallucination was less than one month; and a group of prolonged and continuous type in which the period of duration of delusion or hallucination was one month or more.
  • a GIRK channel gene polymorphism capable of evaluating an individual difference associated with drug sensitivity or disease vulnerability, a method of evaluating drug sensitivity or disease vulnerability using the gene polymorphism and the like can be provided.
  • a proper prescribed amount, a proper prescribed schedule associated with a narcotic drug such as morphine and the like can be easily found, and hence the method is extremely useful for personalized pain therapy, drug dependence therapy and the like.
  • SEQ ID NO: 1 An oligonucleotide containing a gene polymorphism (A-1361G) in GIRK2 subunit gene. r in the nucleotide sequence indicates the gene polymorphism (A-1361G).
  • SEQ ID NO: 2 An oligonucleotide containing a gene polymorphism (G-1250A) in GIRK2 subunit gene. r in the nucleotide sequence indicates the gene polymorphism (G-1250A).
  • SEQ ID NO: 3 An oligonucleotide containing a gene polymorphism (T-244C) in GIRK2 subunit gene. y in the nucleotide sequence indicates the gene polymorphism (T-244C).
  • SEQ ID NO: 4 An oligonucleotide containing a gene polymorphism (C-227T) in GIRK2 subunit gene. y in the nucleotide sequence indicates the gene polymorphism (C-227T).
  • SEQ ID NO: 5 An oligonucleotide containing a gene polymorphism (A-68G) in GIRK2 subunit gene. r in the nucleotide sequence indicates the gene polymorphism (A-68G).
  • SEQ ID NO: 6 An oligonucleotide containing a gene polymorphism (IVS1C75167T) in GIRK2 subunit gene. y in the nucleotide sequence indicates the gene polymorphism (IVS1C75167T).
  • SEQ ID NO: 7 An oligonucleotide containing a gene polymorphism (A1032G) in GIRK2 subunit gene. r in the nucleotide sequence indicates the gene polymorphism (A1032G).
  • SEQ ID NO: 8 An oligonucleotide containing a gene polymorphism (C1569T) in GIRK2 subunit gene. y in the nucleotide sequence indicates the gene polymorphism (C1569T).
  • SEQ ID NO: 9 An oligonucleotide containing a gene polymorphism (C1843G) in GIRK2 subunit gene. s in the nucleotide sequence indicates the gene polymorphism (C1843G).
  • SEQ ID NO: 10 An oligonucleotide containing a gene polymorphism (A-1329C) in GIRK3 subunit gene. m in the nucleotide sequence indicates the gene polymorphism (A-1329C).
  • SEQ ID NO: 11 An oligonucleotide containing a gene polymorphism (C-979G) in GIRK3 subunit gene. s in the nucleotide sequence indicates the gene polymorphism (C-979G).
  • SEQ ID NO: 12 An oligonucleotide containing a gene polymorphism (C-968G) in GIRK3 subunit gene. s in the nucleotide sequence indicates the gene polymorphism (C-968G).
  • SEQ ID NO: 13 An oligonucleotide containing a gene polymorphism (A-447G) in GIRK3 subunit gene. r in the nucleotide sequence indicates the gene polymorphism (A-447G).
  • SEQ ID NO: 14 An oligonucleotide containing a gene polymorphism (C1211T) in GIRK3 subunit gene. y in the nucleotide sequence indicates the gene polymorphism (C1211T).
  • SEQ ID NO: 15 An oligonucleotide containing a gene polymorphism (C1339T) in GIRK3 subunit gene. y in the nucleotide sequence indicates the gene polymorphism (C1339T).
  • SEQ ID NO: 16 An oligonucleotide containing a gene polymorphism (C1781T) in GIRK3 subunit gene. y in the nucleotide sequence indicates the gene polymorphism (C1781T).
  • SEQ ID NO: 17 An oligonucleotide containing a gene polymorphism (C1817T) in GIRK3 subunit gene. y in the nucleotide sequence indicates the gene polymorphism (C1817T).
  • SEQ ID NO: 18 An oligonucleotide containing a gene polymorphism (G2069A) in GIRK3 subunit gene. r in the nucleotide sequence indicates the gene polymorphism (G2069A).
  • SEQ ID NO: 19 An oligonucleotide containing a gene polymorphism (C2429T) in GIRK3 subunit gene. y in the nucleotide sequence indicates the gene polymorphism (C2429T).
  • SEQ ID NO: 20 A nucleotide sequence of a primer for detecting a gene polymorphism (G-1250A) in GIRK2 subunit gene.
  • SEQ ID NO: 21 A nucleotide sequence of a primer for detecting a gene polymorphism (G-1250A) in GIRK2 subunit gene.
  • SEQ ID NO: 22 A nucleotide sequence of a primer for detecting a gene polymorphism (A1032G) in GIRK2 subunit gene.
  • SEQ ID NO: 23 A nucleotide sequence of a primer for detecting a gene polymorphism (A1032G) in GIRK2 subunit gene.
  • SEQ ID NO: 24 A nucleotide sequence of a primer for detecting a gene polymorphism (C1339T) in GIRK3 subunit gene.
  • SEQ ID NO: 25 A nucleotide sequence of a primer for detecting a gene polymorphism (C1339T) in GIRK3 subunit gene.

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EP3110968B1 (de) 2014-02-24 2019-04-17 Children's Hospital Medical Center Verfahren und zusammensetzungen zur personalisierten schmerzbekämpfung
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CN108962339A (zh) * 2018-06-11 2018-12-07 山东中医药大学附属医院 基因多态性与血脂水平的关联性对照方法

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